Increased prevalence of methicillin-resistant Staphylococcus aureus nasal colonization in household contacts of children with community acquired disease

This was a cross sectional study performed at Children's Hospital of Michigan (Detroit, MI). The study was approved by the Institutional Review Board at Wayne State University. Informed consent was obtained from all participants/legal guardians. The study group consisted of all household contacts of patients aged less than 21 years with CA-MRSA infections who were admitted to our hospital during the period October 1, 2007 to October 30, 2008. The control group consisted of patients without suspected staphylococcal infections admitted into our hospital and all their household contacts during the same time period. CA-MRSA infection was defined as infection caused by MRSA isolate cultured within 48 hours of admission. Participants in the study group were identified through prospective monitoring of the daily admission census and the culture results of the microbiology laboratory. For each patient with CA-MRSA infection enrolled, another patient of similar age without a suspected staphylococcal infection and not receiving antibiotics was identified and enrolled with all household contacts.

After obtaining the appropriate consent, guardians of each study subject were interviewed by a study investigator. Data collected, included age, gender, ethnicity, the primary job of the working household member, any history of recent hospitalization, surgery, dialysis, a permanent indwelling catheter or percutaneous medical device, a positive culture for MRSA prior to this infection, history of recurrent soft tissue infection, antibiotic use, residence in a long -term care facility within the previous 12 months for patients and household contacts, sport or gym participation and volunteer time at a health related facility or day care center. Antibiotic susceptibility results of the all CA-MRSA isolates were also recorded. Based on recent published data [21], we hypothesized that the prevalence of CA-MRSA nasal colonization will be 20% in the household contacts of the CA-MRSA infected patients and 5% in the control group. Based upon this proportional effect size difference a sample size of 76 subjects in each study group would provide power of 80.5% with alpha set at 0.05, two-tailed. Sample Power Version 2.0 was used to calculate the sample size.

A non-parametric Fisher's Exact test was used to examine the difference in colonization rates between household members of patients with CA-MRSA infection and those in the control group. All statistical procedures were conducted using SPSS Version 15.0. To examine possible predictor variables of patients with CA-MRSA infections, as opposed to those patients who do not have the infection, a series of univariate and multivariate tests were conducted.

Using moistened double cotton swabs [(BBL CultureSwab Collection and Transport System; Becton, Dickinson and Company, Spark, MD, USA)], cultures were obtained from both anterior nares of each participant. For children with CA-MRSA infections, nasal swabs were obtained soon after identification of culture results from primary site of infection; all had received at least 48 hrs of antibiotic therapy prior to obtaining cultures. Staphylococcus aureus strain identification and antibiotic susceptibility testing were performed using standard laboratory procedures, including colonial morphology, gram stain, catalase test, tube coagulase test of citrated rabbit plasma, and the biochemical reactions in the Microscan Walk-Away (W. Sacramento CA, USA). DNA was extracted from MRSA (infective and nasal) isolates using UltraClean Microbial DNA isolation kit (Mo Bio laboratories, Solana Beach, Calif.). The multiplex PCR for mec element type assignment was performed according to the protocol developed by Oliveira et al. [23]. Detection of PVL genes, LukS-PV and LukF-PV was performed by PCR using primers described by Lina et al. [24]. S. aureus isolates were evaluated in Pulse Field Gel Electrophoresis (PFGE) using SmaI-digested DNA, as described previously [25]. Gels were run at 6 V/cm, 14°C, at an included angle of 120°, on a 1.2% agarose gel with pulse times of 5-35 sec for 21 hrs and strain relatedness was determined by visual inspection of the gel using the criteria of Tenover et al. [26], and dice's coefficient using BioNumerics Software (Version 4.6, Applied Maths, Saint-Martens-Latem, Belgium).